Applications for estrone in preparing anti-ovarian cancer and/or breast cancer products

ABSTRACT

This invention discloses uses for estrone in preparing anti-ovarian cancer and/or breast cancer products. This invention provides uses for estrone in the preparation of products to treat ovarian cancer and/or breast cancer. From carrying out cancer drug repositioning for the FDA- and CFDA-approved drug estrone, experiments for this invention show, based on screening of non-anti-cancer drugs for various cancer cell lines (tissue types) and mutation sites, that estrone has a new use as an anti-ovarian cancer and/or anti-breast cancer medication, thus achieving a new purpose for an old drug.

TECHNICAL FIELD

The present invention relates to the technical field of biology, and it particularly relates to the application of estrone in the preparation of anti-ovarian cancer and/or breast cancer products.

BACKGROUND

Cancer is the most common as well as the most serious disease that threatens human health, and developing effective anti-cancer medications is critical to extending patients' lives. Along with the rapid development of cancer genomics and molecular pharmacology in recent years, the development of new anti-cancer medications has had relatively good outcomes. However, since the bottlenecks of large investments required in the development of new medications and the long-time periods cannot be overcome, as well as the great individual variation in tumor genetics, many traditional anti-cancer medications are not very effective, new medications are expensive, and side effects are not well understood.

In a paper published by the researchers Barabasi A L et. al. in the 2011 Nature Reviews Genetics, a molecular network analysis conducted based on GWAS findings and an interactome strategy is expected to reveal new drug targets and molecular markers for complex diseases, and ultimately to provide an entirely new understanding of disease pathogenesis and treatment approaches. Even more noteworthy is that it has been discovered in drug repositioning studies that susceptibility genes locked in by GWAS studies as well as their genes with protein-protein interaction (PPI) can more easily become indirect targets for medications. This discovery aids in explaining the mechanisms of action of currently available drugs as well as guiding new drug research. In 2014, researchers Okada Y et. al. published a paper in Nature showing that out of the 101 susceptibility genes for rheumatoid arthritis found through a meta-analysis of GWAS findings, 98 are currently being used as direct or indirect targets for rheumatoid arthritis medications. They also discovered through drug repositioning research that there are dozens of medications that have been approved for use for other indications that could be used to treat rheumatoid arthritis.

DISCLOSURE

This research was carried out through integrating cancer gene profiles of the Cancer Gene Census of the Cosmic version 72 cancer histological database as well as the protein interactions in the STRING version 10 database with Drug Bank Version 4.2, the database of FDA approved medications. This obtained candidates for drug repositioning and screening tests for tumor cell lines were carried out, revealing new anti-cancer drugs. Candidates for tumor suppressing drugs revealed from the cancer cell line screening are as follows:

nicardipine, promethazine, estrone, sulindac, etonogestrel, levonorgestrel, mesalazine, indomethacin, sulfasalazine, palsalazide, irbesartan, ibuprofen, isoprenaline, and pentosan polysulfate.

The primary goal of this invention is to provide a new use for estrone.

This invention provides uses for estrone in the preparation of products to treat ovarian cancer and/or breast cancer.

The second goal of this invention is to provide a new use for estrone.

This invention provides uses for estrone in the preparation of products to inhibit the proliferation of ovarian cancer cells and/or breast cancer cells.

The third goal of this invention is to provide a new use for estrone.

This invention provides uses for estrone in the preparation of products to reduce IC50 values in ovarian cancer cells and/or breast cancer cells.

Uses of estrone in treating ovarian cancer and/or breast cancer are also within scope of protection of this invention.

Uses of estrone in inhibiting the proliferation of ovarian cancer cells and/or breast cancer cells are also within scope of protection of this invention.

Uses of estrone as a medication for treating ovarian cancer and/or breast cancer are also within scope of protection of this invention;

Uses of estrone as a medication for inhibiting the proliferation of ovarian cancer cells and/or breast cancer cells are also within scope of protection of this invention.

In the application above, the ovarian cancer cells mentioned are SKOV-3; the breast cancer cells mentioned are HCC1395.

In the uses above, the product is a medication or reagent kit.

The fourth goal of this invention is to provide a kind of product.

The active ingredient in the product of this invention is Estrone, and it has at least one of the following functions:

1) Treatment of ovarian cancer and/or breast cancer;

2) Inhibition of the proliferation of ovarian cancer cells and/or breast cancer cells;

3) Reduction of IC50 values of ovarian cancer cells and/or breast cancer cells;

In the products described above, the ovarian cancer cells mentioned are SKOV-3; the breast cancer cells mentioned are HCC1395.

In the product above, the product is a medication or reagent kit.

BRIEF DESCRIPTION OF THE DRAWINGS

FIG. 1 is a distributed 96-well drug screening culture plate.

FIG. 2 is estrone sensitivity to ovarian cancer; EC50=16.4284; IC50=21.5327; R²=0.9875.

FIG. 3 is estrone sensitivity to breast cancer; EC50=74037.5043; IC50=67.9510; R²=0.9909.

BEST MODE TO CARRY OUT THE INVENTION

Unless otherwise specified, the experimental methods employed in the following examples are standard methods.

Materials, reagents, etc. used in the following examples are all commercially available unless otherwise specified, and the experimental methods employed in the following examples are standard methods.

The analyte drug in the following examples is Estrone, and its chemical composition is as follows:

It is a drug bank product with a catalog number of DB00655.

In the examples below, the product sources for the SKOV-3 ovarian cancer cells, the NCI-H1437 human lung cancer cells, the NCI-H460 large-cell lung cancer cells, and the HCC1395 breast cancer cells are as follows:

SKOV-3 ATCC HTB-77

NCI-H1437 ATCC CRL-5872

NCI-H460 ATCC HTB-177

HCC1395 ATCC CRL-2324

The primary instruments and materials in the examples below are:

DMSO (from Sigma, Cat. No. D4540)

96-well clear bottom cell culture plates (from Corning, Cat. No. 3610)

CellTiter Glo reagent kit (from Promega, Cat. No. G7573)

Doxorubicin positive medication (from MCE, Cat. No. HY-15142)

Fetal Bovine Serum (from Gibco, Cat #10099141)

100 mm petri dish (from Corning, Cat #430167)

RPMI-1640 medium (from Gibco, Cat #A1049101)

DMEM medium (from Gibco, Cat #11995081)

DMEM/F12 medium (from Gibco, Cat #11330057)

EMEM medium (from Gibco, Cat #10370021)

Multidrop 384 cell dispensers (Thermo, Cat #5840150)

EnSpire multi-function plate reader (Perkin Elmer, Cat #2300-001M)

In example 1, CELLTITER-GLO was used to test estrone against ovarian cancer and/or breast cancer

A. Test Plate Preparation

1. Cell plating

a) The complete medium required for each cell was prepared.

b) Before beginning the experiment, the name of the drug screened for the cells marked on the 100 mm petri dish was confirmed as well as information such as the passage time and number of passages to ensure the experiment was error-free.

c) Refer to steps d) through i) for procedures for adherent cells; refer to steps j) through l) for procedures for suspension cells.

d) When using aseptic technique, a vacuum pump was used to draw the cell culture medium.

e) 2 ml of a sterile PBS solution was used to rinse the cell surface, and a vacuum pump was used to aspirate the PBS waste.

f) A 1 ml 0.25% (w/v) Trypsin-0.038% (w/v) EDTA solution was gently added to the petri dish for cell digestion, and after gently mixing several times, the solution covered the cell surfaces. The status of cell digestion was observed under an inverted microscope, and the trypsin digestion effect was terminated when cell shedding was about to occur.

g) 5 ml of pre-warmed 37° C. complete medium was added to the petri dishes, and a pipette was used to gently dissociate the cells in order for them to shed from the bottom of the petri dish.

h) The cells were suspended and transferred to a 15 ml or 50 ml sterile centrifuge tube and they were centrifuged at 1000 rpm for 5 minutes.

i) A vacuum pump was used to aspirate the medium with aseptic technique. 5 ml of pre-warmed 37° C. complete medium was used to resuspend the cell sediment, and it was gently dissociated to mix evenly.

j) A pipette was used to gently dissociate the cells so that they fully shed from the bottom of the petri dish.

k) The cells were suspended and transferred to a 15 ml or 50 ml sterile centrifuge tube and they were centrifuged at 1000 rpm for 5 minutes.

l) A vacuum pump was used to aspirate the medium with aseptic technique. 5 ml of pre-warmed 37° C. complete medium was used to resuspend the cell sediment, and it was gently dissociated to mix evenly.

m) A cell counter was used to count the number of suspended cells and adjust the cell suspension to an appropriate density in the plate to carry out cell plating experiments.

SKOV-3 cells were handled as described above, and a SKOV-3 96-well cell culture plate was obtained.

The complete medium for SKOV-3 cells was McCOY'S 5A (a live product), Cat #16600082, with a cells/well density of 12000.

2. The drug analyte estrone was prepared and administered (200× final concentration):

1) The master plate for the drug analyte estrone was prepared

a) DMSO was used to dilute the analyte estrone to 20 mM for use.

b) 79 μL of the 20 mM analyte prepared in step a) was added to the first well in the first row of the dilution plate, and then 54 μL of DMSO solution was added to the second through ninth wells of the first row. 25 μL of solution was aspirated from the first to the second well, and after mixing well 25 μL of solution was aspirated from the second to the third well, and this was repeated until the 9th well in order to ensure that 3.16 dilution of the medication would be carried out one-by-one.

2) Doxorubicin positive medication (MCE, Cat. No. HY-15142) master plate preparation

a) DMSO was used to dilute Doxorubicin positive medication to 6 mM for use.

b) The 6 mM Doxorubicin positive medication solution was added to the dilution plate, and the DMSO solution was incrementally added to the analyte medication to 1:3.16.

3. Drug working board preparation and dosing

a) The analyte drug and the positive drug sampling template is as shown in FIG. 1, in which S1208: Positive medication Doxorubicin, DMSO: Positive control well, Cpd 1, 2, 3: Analyte drug, DMSO final concentration of 0.5% (DMSO compatibility).

b) 95 μl of cell-specific complete medium was added to the working plate, each medication to 9 wells. A multi-channel pipettor was used to transfer a series of 5 μl (9 wells) of the diluted solution of the analyte drug and positive medication Doxorubicin (10× final concentration) from the working plate, achieving cell culture media of varying concentrations.

c) The SKOV-3 96-well cell plates prepared in step 1 were removed from the incubator, and 10 μl of the cell culture media (10× final concentration) with varying drug concentrations as described in b) above was added to the SKOV-3 96-well cell culture plate row-by-row as shown in FIG. 1. It was placed into a CO₂ incubator at 37° C. for 72 hours, obtaining the SKOV-3 96-well drug screening plate.

Wells with no medication added acted as controls.

The final concentration and dosing of the analyte drug, positive medication Doxorubicin, and control in the 96-well plates were as follows:

The final concentrations (μM) of the analyte drug in wells 2-10 in FIG. 1 are, in order: 100, 31.64557, 10.01442, 3.16912, 1.002886, 0.317369, 0.100433, 0.031783, 0.010058;

The final concentration (μM) of the positive medication Doxorubicin in wells 2-10 in FIG. 1 are, in order: 30, 9.493671, 3.004326, 0.950736, 0.300866, 0.095211, 0.03013, 0.009535, 0.003017;

In addition, the S1208 well in the 96-well plate (E1-H1 and A12-D12): 10 μl of the final concentration 100 μM Doxorubicin solution (solvent containing 0.5% DMSO complete culture medium solution), DMSO wells (A1-D1, E12-H12, and A11-H11): 10 μl containing 0.5% DMSO complete culture medium solution.

B. CELLTITER-GLO Luminescent Cell Viability Assay System

1. CellTiter-Glo reagent preparation

a) The CellTiter-Glo reagent buffer was thawed before using and stabilized to room temperature for use.

b) The CellTiter-Glo reagent frozen substrate was thawed before using and stabilized to room temperature for use.

c) 100 ml of stabilized CellTiter-Glo buffer was added to the container with CellTiter-Glo reagent frozen substrate to adequately resuspend it to form an enzyme/substrate mixture, also referred to as the CellTiter-Glo assay reagent.

d) It was gently mixed and vortexed and inverted multiple times to achieve a uniform solution. In general, the CellTiter-Glo substrate reagent will adequately dissolve within 1 minute. It is stored separately in low-light conditions at −20° C. to await use, and freezing repeatedly should be avoided.

2. Testing

a) Before testing, the SKOV-3 96-well drug screening plate described in 3 above was stabilized to room temperature for 20-30 minutes.

b) An inverted microscope was used to observe the conditions of each group of cells in the culture plate and their death patterns, and any abnormal conditions were noted and retested.

c) 100 μl of CellTiter-Glo reagent (prepared as described in 1 above) was added to all drug screening plates and mixed evenly.

d) It was thoroughly oscillated in a 96-well microplate oscillator for 2 minutes to allow the cells to undergo full lysis.

e) It was stored away from light at room temperature for 15 minutes before carrying out luminescent signal detection to ensure signal stability.

f) An EnSpire multi-function plate reader was used at 570 nm to read the luminescent signals.

g) Data was processed and analyzed.

The results of the SKOV-3 96-well drug screening plate are shown in FIG. 2.

The IC50 value was calculated; results are shown in Table 1.

The same method was used to test Estrone's action on the IC50 value of HCC1395 breast cancer cells; results are shown in Table 1 and FIG. 3.

Breast cancer cells HCC1395, complete medium basis of RPMI-1640, (a live product), Cat #A1049101, with a cells/well density of 6000.

The same method was used to test Estrone's action on the IC50 value of NCI-H460 human lung cancer cells and NCI-H460 large-cell lung cancer cells; results are shown in Table 1.

It is evident that estrone has a specific inhibitory effect on the proliferation of ovarian cancer cells and it can be used as a medication for ovarian cancer treatment.

TABLE 1 IC50 values of various cells under the effect of Estrone Cells IC50 value SKOV-3 21.5327 NCI-H460 100 NCI-H1437 100 HCC1395 67.9510

INDUSTRIAL APPLICATIONS

From carrying out cancer drug repositioning for the FDA- and CFDA-approved drug Estrone, experiments for this invention show, based on screening of non-anti-cancer drugs for various cancer cell lines (tissue types) and mutation sites, that estrone has a new use as an anti-ovarian cancer and/or anti-breast cancer medication, thus achieving a new purpose for an old drug. 

1-9. (canceled)
 10. A method for treating ovarian cancer in a subject comprising administering an effective amount of estrone to the subject.
 11. A method for inhibiting the proliferation of ovarian cancer cells comprising contacting the cells with an effective amount of estrone.
 12. The method of claim 11, wherein the ovarian cancer cells are SKOV-3.
 13. The method of claim 10, wherein the subject is a human patient. 